Structural and functional characterization of the pore-forming domain of pinholin S2168

Author:

Steger Lena M. E.ORCID,Kohlmeyer AnnikaORCID,Wadhwani ParveshORCID,Bürck JochenORCID,Strandberg ErikORCID,Reichert Johannes,Grage Stephan L.ORCID,Afonin SergiiORCID,Kempfer MarinORCID,Görner Anne C.,Koch JuliaORCID,Walther Torsten H.ORCID,Ulrich Anne S.ORCID

Abstract

Pinholin S2168 triggers the lytic cycle of bacteriophage φ21 in infectedEscherichia coli. Activated transmembrane dimers oligomerize into small holes and uncouple the proton gradient. Transmembrane domain 1 (TMD1) regulates this activity, while TMD2 is postulated to form the actual “pinholes.” Focusing on the TMD2 fragment, we used synchrotron radiation-based circular dichroism to confirm its α-helical conformation and transmembrane alignment. Solid-state15N-NMR in oriented DMPC bilayers yielded a helix tilt angle of τ = 14°, a high order parameter (Smol= 0.9), and revealed the azimuthal angle. The resulting rotational orientation places an extended glycine zipper motif (G40xxxS44xxxG48) together with a patch of H-bonding residues (T51, T54, N55) sideways along TMD2, available for helix–helix interactions. Using fluorescence vesicle leakage assays, we demonstrate that TMD2 forms stable holes with an estimated diameter of 2 nm, as long as the glycine zipper motif remains intact. Based on our experimental data, we suggest structural models for the oligomeric pinhole (right-handed heptameric TMD2 bundle), for the active dimer (right-handed Gly-zipped TMD2/TMD2 dimer), and for the full-length pinholin protein before being triggered (Gly-zipped TMD2/TMD1-TMD1/TMD2 dimer in a line).

Funder

Deutsche Forschungsgemeinschaft

Helmholtz-Gemeinschaft

Publisher

Proceedings of the National Academy of Sciences

Subject

Multidisciplinary

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